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Determining the N-terminal orientations of recombinant transmembrane proteins in the Escherichia coli plasma membrane

机译:测定大肠杆菌质膜中重组跨膜蛋白的N端方向

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摘要

In silico algorithms have been the common approach for transmembrane (TM) protein topology prediction. However, computational tools may produce questionable results and experimental validation has proven difficult. Although biochemical strategies are available to determine the C-terminal orientation of TM proteins, experimental strategies to determine the N-terminal orientation are still limited but needed because the N-terminal end is essential for membrane targeting. Here, we describe a new and easy method to effectively determine the N-terminal orientation of the target TM proteins in Escherichia coli plasma membrane environment. D94N, the mutant of bacteriorhodopsin from Haloarcula marismortui , can be a fusion partner to increase the production of the target TM proteins if their N-termini are in cytoplasm (Nin orientation). To create a suitable linker for orientating the target TM proteins with the periplasmic N-termini (Nout orientation) correctly, we designed a three-TM-helix linker fused at the C-terminus of D94N fusion partner (termed D94N-3TM) and found that D94N-3TM can specifically improve the production of the Nout target TM proteins. In conclusion, D94N and D94N-3TM fusion partners can be applied to determine the N-terminal end of the target TM proteins oriented either Nin or Nout by evaluating the net expression of the fusion proteins.
机译:电子计算机算法已成为跨膜(TM)蛋白质拓扑预测的常用方法。但是,计算工具可能会产生可疑的结果,并且已经证明实验验证很困难。尽管生物化学策略可用于确定TM蛋白的C端方向,但确定N端方向的实验策略仍然有限,但由于N端对于膜靶向必不可少,因此仍是必需的。在这里,我们描述了一种新的简便方法,可以有效地确定大肠杆菌质膜环境中目标TM蛋白的N端方向。如果D94N是一种来自细菌嗜盐菌的细菌视紫红质的突变体,则如果其N末端在细胞质中(N 方向),则可以作为融合伴侣以增加目标TM蛋白的产量。为了创建合适的接头来正确定向带有周质N末端(N out 方向)的目标TM蛋白,我们设计了一个在D94N融合伴侣C端融合的3-TM-螺旋接头(称为D94N-3TM),发现D94N-3TM可以特异性提高N out 靶TM蛋白的产生。总之,D94N和D94N-3TM融合伴侣可以通过评估净值来确定定向为N in 或N out 的目标TM蛋白的N末端。融合蛋白的表达。

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